藜CaMAPKK2的表达分析及盐胁迫信号通路互作组分的筛选  被引量：2

作　　者：陈莎莎[1] 贺转转[1] 姜生秀[1] 李晓荣[1] 邢佳佳[1] 吕秀云[1] 兰海燕[1] 

机构地区：[1]新疆大学生命科学与技术学院/新疆生物资源基因工程重点实验室,乌鲁木齐830046

出　　处：《中国农业科学》2013年第5期889-897,共9页Scientia Agricultura Sinica

基　　金：国家科技部"973"前期项目(2012CB722204);国家自然科学基金(30660012);新疆自治区科技攻关重大专项(200731138-3);新疆生物资源与基因工程重点实验室开放基金(XJDX0201-2007-03;XJDX0201-2009-06)

摘　　要：【目的】通过对抗逆植物藜的丝裂原活化蛋白激酶(MAPK)级联途径中MAPKK的胁迫表达模式分析及信号转导途径互作组分的筛选,探索植物藜响应外界胁迫信号诱发逆境耐受的机制。【方法】以藜叶片总RNA为模板,利用定量PCR方法对NaCl、H2O2和ABA胁迫下藜MAPKK表达规律进行了分析。利用RT-PCR结合RACE技术获得了藜MAPKK的全长cDNA序列。利用酵母双杂交技术对MAPKK盐胁迫信号通路互作组分进行了分析。【结果】获得一个藜MAPKK的全长cDNA序列,命名为CaMAPKK2,其开放阅读框为1 089 bp,编码一个由362个氨基酸组成的丝裂原活化蛋白激酶。定量PCR显示CaMAPKK2受盐胁迫诱导明显上调表达,同时受外源H2O2和ABA调控。H2O2合成抑制剂DPI与ABA合成抑制剂Na2WO4显著抑制了300 mmol.L-1NaCl处理下CaMAPKK2的表达。以全长CaMAPKK2为诱饵蛋白,利用酵母双杂交技术筛选到5个可能与CaMAPKK2相互作用的蛋白。测序结果显示,其中1个序列可通读,该cDNA序列长794 bp,与欧洲赤杨(Alnus glutinosa)和拟南芥的噻唑合成酶(thiazole biosyntheticenzyme)基因AgTHI1和AtTHI1核酸序列相似度达79%和78%,其它4个序列没有连续的读码框。【结论】CaMAPKK2受NaCl和H2O2诱导上调表达,暗示盐胁迫可能通过诱导H2O2和ABA的积累从而导致CaMAPKK2表达增加。要进一步筛选CaMAPKK2互作组分需获得更多阳性克隆并开展相关功能验证试验。[ Objective ] The aim of the present study is to understand the mechanism of stress signal transduction to induce the response of adverse tolerance with Chenopodium album, an adverse-tolerant plant species, through analysis of the expression pattern of mitogen-activated protein kinase gene （MAPKK） under different abiotic stresses and screening of interaction proteins of MAPKK in MAPK signal transduction pathways. [Method] Using the total RNA from the leafofC, album as the template, the expression patterns of MAPKK under NaC1, H202 and ABA were analyzed by quantitative PCR technique. The full-length cDNA sequence of MAPKK was obtained by combined reverse transcription-PCR （RT-PCR） and RACE techniques. The yeast two-hybrid technique was employed to analyze the interaction components of MAPKK in salt-stress signal pathway. [Result] A full length cDNA fragment of MAPKK gene from C. album included a 1 089 bp ORF, which encodes with 362 putative amino acids, named as CaMAPKK2. qPCR analysis showed that CaMAPKK2 gene was significantly induced by salt and H202 but not by ABA stress, at least in the present study.DPI or Na2WO4 （inhibitor of H2O2 or ABA synthesis） significantly inhibited the expression of CaMAPKK2 in C. album when exposed to 300 mmol.L-1 NaCl stress. By using the CaMAPKK2 as bait protein, five potential clones which may interact with CaMAPKK2 were obtained by the first screening of yeast two hybridization. Sequencing result indicated that one 794 bp fragment out of 5 eDNA showed correct reading frame, and shared identities of 79% and 78% in nucleotide sequence to ~4gTHI1 and AtTH11 （thiazole biosynthetic enzyme） from Alnus glutinosa and Arabidopsis thaliana, respectively, while other 4 eDNA sequences had no correct reading frame. [Conclusion] CaMAPKK2 gene was significantly induced by salt and 1-1202 stress, suggesting that salt stress might induce the accumulation of H202 and ABA, which in turn leads to expression increasing of MAPKK. More positive clones should be acquired and the relevan

关 键 词：藜 盐胁迫 信号转导途径 MAPKK 酵母双杂交 定量PCR 

分 类 号：Q943[生物学—植物学]